A Simple and Highly Sensitive Liquid Chromatographic-Mass Spectrometric Method for the Determination of Itraconazole and Its Major Metabolite in Human Plasma and Its Application to a Bioequivalence Study.

IF 1.3 4区 化学 Q4 BIOCHEMICAL RESEARCH METHODS
Hamed Hamishehkar, Rasoul Hosseinpour, Ladan Dayani, Bahareh Samii, Jaber Emami
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引用次数: 0

Abstract

Itraconazole is an oral triazole antimycotic drug. Bioequivalence studies are cornerstones for the approval of generic drug development globally. The present study describes a simple, sensitive and economical LC-MS/MS method for the determination of itraconazole and its metabolite in human plasma. Itraconazole (drug), hydroxyitraconazole (metabolite), and atorvastatin as internal standard were added to plasma samples. The standard curve of both the drug and metabolite covering the 4-320 ng/mL concentration range, was linear (R2 = 0.999). Also, a limit of quantification of 4 ng/mL of a sample size of 0.4 mL is achieved which is comparable or even better than the reported methods. The applicability of this method was proven by analyzing true samples obtained after the administration of 100 mg itraconazole of test (Noxifunge®) and reference (Sporanox®) to healthy volunteers. The 90% confidence intervals of the logarithmically transformed AUC0-72, AUC0-∞, and Cmax of the two formulations both for the drug and the metabolite are within the accepted levels proposed by FDA and EMA. Therefore, the presented method is suitable for bioavailability, pharmacokinetic, and bioequivalent studies in humans.

高效液相色谱-质谱联用法测定人血浆中伊曲康唑及其主要代谢物及其生物等效性研究
伊曲康唑是一种口服三唑类抗真菌药物。生物等效性研究是全球仿制药开发批准的基石。建立了一种简便、灵敏、经济的hplc -MS/MS法测定人血浆中伊曲康唑及其代谢物的含量。血浆样品中加入伊曲康唑(药物)、羟伊曲康唑(代谢物)和阿托伐他汀作为内标。在4 ~ 320 ng/mL浓度范围内,药物与代谢物的标准曲线均呈良好的线性关系(R2 = 0.999)。此外,定量限为4 ng/mL,样本量为0.4 mL,这与报道的方法相当,甚至更好。通过对健康志愿者服用100mg伊曲康唑(试验品(noxfunge®)和参比品(Sporanox®)后获得的真实样品进行分析,证明了该方法的适用性。两种制剂对药物和代谢物的对数变换后的AUC0-72、AUC0-∞和Cmax的90%置信区间均在FDA和EMA提出的可接受水平之内。因此,该方法适用于人类的生物利用度、药代动力学和生物等效性研究。
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来源期刊
CiteScore
2.90
自引率
7.70%
发文量
94
审稿时长
5.6 months
期刊介绍: The Journal of Chromatographic Science is devoted to the dissemination of information concerning all methods of chromatographic analysis. The standard manuscript is a description of recent original research that covers any or all phases of a specific separation problem, principle, or method. Manuscripts which have a high degree of novelty and fundamental significance to the field of separation science are particularly encouraged. It is expected the authors will clearly state in the Introduction how their method compares in some markedly new and improved way to previous published related methods. Analytical performance characteristics of new methods including sensitivity, tested limits of detection or quantification, accuracy, precision, and specificity should be provided. Manuscripts which describe a straightforward extension of a known analytical method or an application to a previously analyzed and/or uncomplicated sample matrix will not normally be reviewed favorably. Manuscripts in which mass spectrometry is the dominant analytical method and chromatography is of marked secondary importance may be declined.
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